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建立了用高效液相色谱(HPLC)-二极管阵列检测器(DAD)测定化妆品中两种呋喃香豆素同分异构体-8-甲氧基补骨脂素(8-MOP)和5-甲氧基补骨脂素(5-MOP)的简便方法。样品用甲醇超声提取,高速冷冻离心,经0.45μm滤膜过滤,注入高效液相色谱,用DAD进行扫描检测,并在301 nm波长进行分析。用保留时间结合紫外光谱图定性,外标法定量,并且采用液质联用(LC/MS/MS)确证。测试结果对8-MOP的回收率为87.0%~105.0%,RSD为0.41%~5.3%,检出限为5.0 mg/kg;5-MOP的回收率为88.0%~105.0%,RSD为0.33%~4.1%,检出限为5.0 mg/kg。本文用DAD同时分离和检测了化妆品中的8-MOP和5-MOP,方法可用于化妆品安全性监控。 相似文献
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建立了高效液相色谱(HPLC)/二极管阵列检测器(DAD)测定化妆品中甲氨蝶呤的方法. 乳液、膏霜、化妆水、散粉、唇膏类等不同类型的化妆品样品经超声提取后, 高效液相色谱DAD 扫描检测, 并在302 nm进行分析. 用保留时间结合紫外光谱定性, 外标法定量. 甲氨蝶呤在0.05~100 mg/L的范围内线性关系良好(r=0.9999). 在添加质量浓度为0.05~1.0 mg/L范围时, 回收率在87.8%~103.4%之间, 相对标准偏差在0.42%~6.8%, 检出限为0.02 mg/L, 定量限为0.05 mg/L. 该法可用于化妆品中甲氨蝶呤的检测. 相似文献
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建立了高效液相色谱(HPLC)-二极管阵列检测器(DAD)测定化妆品中士的宁和马钱子碱的方法.膏霜、水剂、散粉、香波、唇膏等不同类型的化妆品样品经超声提取后,高效液相色谱-二极管阵列扫描检测,并在264 nm波长进行分析.用保留时间结合紫外光谱定性,外标法定量,并且采用液相色谱-质谱确证.士的宁的回收率为89.2%~103.5%,相对标准偏差在0.7%~6.0%之间,定量限为2.5 mg/kg,马钱子碱的回收率为86.3%~101.0%,相对标准偏差在0.9%~6.9%之间,定量限为2.5 mg/kg. 相似文献
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建立了化妆品中致敏原香豆素及其7种衍生物(二氢香豆素、7-甲氧基香豆素、7-甲基香豆素、7-乙氧基-4-甲基香豆素、环香豆素、双香豆素和醋硝香豆素)的高效液相色谱测定方法。样品以0.1 mol/L氢氧化钠溶液-乙腈(1∶9,体积比)混合溶液进行超声提取,提取液经高速离心及微孔滤膜过滤后,ZORBAX SB-C18(250 mm×4.6 mm,5μm)色谱柱分离,0.05 mol/L乙酸铵溶液(含0.25%乙酸)和乙腈为流动相梯度洗脱,二极管阵列检测器检测,外标法定量。疑似阳性样品采用高效液相色谱-串联质谱法进行确证。结果表明,香豆素及其衍生物在一定浓度范围内线性良好(r2≥0.999 6),定量下限为8~20 mg/kg。在低、中、高3个加标水平下,香豆素及其衍生物的平均回收率为84.6%~100.7%,相对标准偏差(n=6)为0.8%~9.7%。该方法准确、稳定性好、特异性强,能够为化妆品检验和日常生产质量控制提供科学依据及技术支持。 相似文献
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建立了用二极管阵列检测器扫描紫外最大吸收波长,用高效液相色谱紫外检测器测定甲苯法生产己内酰胺精制单元副产物的方法.检测紫外最大吸收波长时使用Lichrospher C18柱(250 mm×4.5 mm i.d.,5μm),流动相为65%的甲醇水溶液,流速0.7 mL/min;定性定量使用Agilent Hypersil ODS C18柱(5μm4.0×250 mm),检测波长215 nm,流动相为V(甲醇):V(水)=38:62溶液,磷酸调节pH为5,流速0.4 mL/min.经理论推导,用保留时间结合各物质的紫外光谱定性,外标法定量.确定该副产物中主要含有环已胺、已内酰胺、苯甲酰胺、环己甲酰胺.环己胺的回收率为98%~99%,精密度为O.23%~1.51%,定量下限为0.05 mg;己内酰胺的回收率为98%~100%,精密度为0.51%~1.63%,定量下限为0.03 mg;苯甲酰胺的回收率为100%~101%,精密度为0.52%~2.02%,定量下限为0.03 mg;环己甲酰胺的回收率为97%~100%.精密度为0.73%~1.25%,定量下限为0.04 mg. 相似文献
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高效液相色谱二极管阵列检测器测定化妆品中的6种酞酸酯 总被引:14,自引:0,他引:14
建立了用高效液相色谱二极管阵列检测器测定化妆品中6种酞酸酯——邻苯二甲酸二甲酯(DMP)、二乙酯(DEP)、二丁酯(DBP)、丁基苄基酯(BBP)、二(2-乙基己)酯(DEHP)和二正辛酯(DOP)的方法一样品用甲醇超声提取.高速冷冻离心,经0.5μm滤膜过滤.直接注入高效液相色谱.在280nm波长进行分析用保留时间结合酞酸酯紫外光谱定性.外标法定量该法的回收率为85%~110%.精密度RSD为0.058%~2.84%.检出限:DMP.DEP、BBP和DBP均为5ng.DEHP和DOP为10ng,该方法准确度和灵敏度高.样品用量少.前处理简单。可同时测定化妆品中6种酞酸酯化合物。 相似文献
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高效液相色谱法对化妆品中17种香豆素类化学成分的同时测定 总被引:2,自引:0,他引:2
建立了同时测定化妆品中17种香豆素类化学成分(双香豆素、7-羟基-6-甲氧基香豆素、8-羟基补骨脂素、香豆素、6,7-二甲氧基香豆素、二氢香豆素、7-甲氧基香豆素、7-甲基香豆素、补骨脂素、8-甲氧基补骨脂素、5-甲氧基补骨脂素、4-甲基-7-乙氧基香豆素、2′,4,8-三甲基补骨脂素、欧前胡素、异欧前胡素、二氢欧山芹醇当归酸酯、环香豆素)的高效液相色谱分析方法。样品经甲醇超声提取,以8 000 r/min离心15 min,取上清液过滤后测定。采用Agilent Zorbax SB-Phenyl柱(4.6 mm×250 mm,5μm)分离,以水-甲醇-乙腈三元流动相梯度洗脱,流速1.0 mL/min,柱温30℃。采用二极管阵列检测器多波长检测(210、220、250 nm),外标法定量。17种香豆素类化合物的定量下限(LOQ)为1 mg/kg,线性范围为0.5~60 mg/L,相关系数(r)均大于0.999。在高、中、低3种加标水平下的平均加标回收率(n=6)为86%~106%,相对标准偏差为0.3%~3.6%。该方法准确、简便,适用于化妆品中17种香豆素类化合物的测定。 相似文献
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建立了同时测定化妆品中8种呋喃香豆素类化合物(8-羟基补骨脂素、补骨脂素、异补骨脂素、8-甲氧基补骨脂素、5-甲氧基补骨脂素、三甲沙林、欧前胡素和异欧前胡素)的高效液相色谱分析方法及液相色谱-串联质谱确证方法。膏霜类、水剂类、香波类、散粉类、唇膏类等不同类型的化妆品样品分别经适宜的提取溶液进行超声提取,提取液以离心处理后,取上清液经微孔滤膜过滤后测定。采用Agilent Zorbax SB-Phenyl色谱柱(250 mm×4.6 mm, 5 μm)分离,以甲醇-乙腈-水三元流动相梯度洗脱,流速1.0 mL/min,柱温30 ℃,检测波长250 nm。8-羟基补骨脂素的定量限为0.25 mg/kg,补骨脂素、异补骨脂素、8-甲氧基补骨脂素、5-甲氧基补骨脂素、三甲沙林、欧前胡素、异欧前胡素的定量限为0.5 mg/kg。在低、中、高3种加标水平下,8种待测组分的平均回收率为85.0%~105.8%,相对标准偏差为0.41%~7.90%。采用本方法在一日内不同时间点(6个时间点,每隔1 h测定一次)和不同日期(6 d内)测定混合标准溶液,得到8个目标物峰面积的日内精密度均小于1%,日间精密度均小于2%。该方法准确、简便、快速,适用于不同类型化妆品中8种呋喃香豆素类化合物的测定。 相似文献
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Parkinson's disease (PD) is a very serious neurological disorder, and current methods of treatment fail to achieve long‐term control. SCH 420814 is a potent, selective and orally active adenosine A2A receptor antagonist discovered by Schering‐Plough. Stability testing provides evidence of the quality of a bulk drug when exposed to the influence of environmental factors. Understanding the drug degradation profiles is critical to the safety and potency assessment of the drug candidate for clinical trials. As a result, identification of degradation products has taken an important role in drug development process. In this study, a rapid and sensitive method was developed for the structural determination of the degradation products of SCH 420814 formed under different forced conditions. The study utilizes a combination of liquid chromatography–tandem‐mass spectrometry (LC‐MS/MS) and Fourier Transform (FT) MS techniques to obtain complementary information for structure elucidation of the unknowns. This combination approach has significant impact on degradation product identification. A total of ten degradation products of SCH 420814 were characterized using the developed method. Copyright © 2009 John Wiley & Sons, Ltd. 相似文献
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《Analytical letters》2012,45(15):1165-1175
Abstract The use of a direct liquid introduction probe with a short guard column as the method of sample introduction is explored. This technique is an alternative to the conventional direct probe method. The method is rapid, involatile compounds can be analyzed, and volatile compounds are not lost in the vacuum lock. Screening for trichlorophenol in urine, by observing the loss of [M-HCOCI]+, is used to test the technique. The advantages and disadvantages of split and splitless direct liquid introduction probes and column concentration are discussed. Detection limits in the low nanograms were observed, and samples may be analyzed every 30 seconds. 相似文献
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In the HPLC of basic drugs and metabolites, good efficiency and peak shape can often be attained using strong cation‐exchange packings with isocratic 100% methanol eluents containing an ionic modifier at an appropriate pH* and ionic strength. Solvent extracts can be analysed directly, and use of ammonium acetate as modifier facilitates the use of atmospheric pressure chemical ionization (APCI)–tandem mass spectrometry, selected reaction monitoring mode. For the analysis of amisulpride and of metamfetamine/amfetamine in plasma (200 µL) after single oral doses in man, a column packed with Waters Spherisorb S5SCX (5 µm average particle size, 100 × 2.1 mm i.d.) was used with methanolic ammonium acetate (40 mmol/L, pH* 6.0, flow rate 0.5 mL/min) as eluent (35°C). Deuterated internal standards were used for each analyte. Detection was by positive‐mode APCI. Responses for all analytes were linear over the calibration ranges. Intra‐assay precision (RSD) was 2–18%, and inter‐assay precision was 2–12%. The limit of detection was 0.5 µg/L for all analytes. No significant matrix effects or isobaric interferences were noted. The total analysis time was 7 min. Similar methodology can be applied to a wide range of basic analytes using MS/MS detection. Copyright © 2010 John Wiley & Sons, Ltd. 相似文献
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乳腺癌代谢物组模式特征发现方法及HPLC/M S/M S分析 总被引:11,自引:0,他引:11
提出一种基于单独最优特征组合和BP神经网络的代谢物组模式特征发现方法,并用其寻找到尿样中与乳腺癌最为相关的4种核苷,组成一组特异性检测参数.经HPLC/MS/MS联用法鉴定,它们是乳清酸核苷、1-甲酰化腺苷、S-腺苷-L-蛋氨酸及N2-甲酰化鸟苷.将这4种核苷作为输入变量,用BP神经分类网络建立乳腺癌诊断模型.留一法交叉验证和独立验证结果表明,该模型预测准确率达到90%以上. 相似文献
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The in vivo and in vitro metabolism of jatrorrhizine has been investigated using a specific and sensitive LC/MS/MS method. In vivo samples including rat feces, urine and plasma collected separately after dosing healthy rats with jatrorrhizine (34 mg/kg) orally, along with in vitro samples prepared by incubating jatrorrhizine with rat intestinal flora and liver microsome, respectively, were purified using a C(18) solid-phase extraction cartridge. The purified samples were then separated with a reversed-phase C(18) column with methanol-formic acid aqueous solution (70:30, v/v, pH3.5) as mobile phase and detected by on-line MS/MS. The structural elucidation of the metabolites was performed by comparing their molecular weights and product ions with those of the parent drug. As a result, seven new metabolites were found in rat urine, 13 metabolites were detected in rat feces, 11 metabolites were detected in rat plasma, 17 metabolites were identified in intestinal flora incubation solution and nine metabolites were detected in liver microsome incubation solution. The main biotransformation reactions of jatrorrhizine were the hydroxylation reaction, the methylation reaction, the demethylation reaction and the dehydrogenation reaction of parent drug and its relative metabolites. All the results were reported for the first time, except for some of the metabolites in rat urine. 相似文献
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Anna C. Crecelius Anja Baumgaertel Ulrich S. Schubert 《Journal of mass spectrometry : JMS》2009,44(9):1277-1286
The detailed characterization of macromolecules plays an important role for synthetic chemists to define and specify the structure and properties of the successfully synthesized polymers. The search for new characterization techniques for polymers is essential for the continuation of the development of improved synthesis methods. The application of tandem mass spectrometry for the detailed characterization of synthetic polymers using the soft ionization techniques matrix‐assisted laser desorption/ionization mass spectrometry (MALDI‐MS) and electrospray ionization mass spectrometry (ESI‐MS), which became the basic tools in proteomics, has greatly been increased in recent years and is summarized in this perspective. Examples of a variety of homopolymers, such as poly(methyl methacrylate), poly(ethylene glycol), as well as copolymers, e.g. copolyesters, are given. The advanced mass spectrometric techniques described in this review will presumably become one of the basic tools in polymer chemistry in the near future. Copyright © 2009 John Wiley & Sons, Ltd. 相似文献
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Streamlined quantitative metabolomics in central metabolism of bacteria would be greatly facilitated by a high-efficiency liquid chromatography (LC) method in conjunction with accurate quantitation. To achieve this goal, a methodology for LC-tandem quadrupole mass spectrometry (LC-MS/MS) involving a pentafluorophenylpropyl (PFPP) column and culture-derived global (13)C-labeled internal standards (I.Ss.) has been developed and compared to hydrophilic interaction liquid chromatography (HILIC)-MS/MS and published combined two-dimensional gas chromatography and LC methods. All 50 tested metabolite standards from 5 classes (amino acids, carboxylic acids, nucleotides, acyl-CoAs and sugar phosphates) displayed good chromatographic separation and sensitivity on the PFPP column. In addition, many important critical pairs such as isomers/isobars (e.g. isoleucine/leucine, methylsuccinic acid/ethylmalonic acid and malonyl-CoA/3-hydroxybutyryl-CoA) and metabolites of similar structure (e.g. malate/fumarate) were resolved better on the PFPP than on the HILIC column. Compared to only one (13)C-labeled I.S., the addition of global (13)C-labeled I.Ss. improved quantitative linearity and accuracy. PFPP-MS/MS with global (13)C-labeled I.Ss. allowed the absolute quantitation of 42 metabolite pool sizes in Methylobacterium extorquens AM1. A comparison of metabolite level changes published previously for ethylamine (C2) versus succinate (C4) cultures of M. extorquens AM1 indicated a good consistency with the data obtained by PFPP-MS/MS, suggesting this single approach has the capability of providing comprehensive metabolite profiling similar to the combination of methods. The more accurate quantification obtained by this method forms a fundamental basis for flux measurements and can be used for metabolism modeling in bacteria in future studies. 相似文献
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